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Annotating and quantifying pri-miRNA transcripts using RNA-Seq data of wild type and serrate-1 globular stage embryos of Arabidopsis thaliana.


ABSTRACT: The genome annotation for the model plant Arabidopsis thaliana does not include the primary transcripts from which MIRNAs are processed. Here we present and analyze the raw mRNA sequencing data from wild type and serrate-1 globular stage embryos of A. thaliana, ecotype Columbia. Because SERRATE is required for pri-miRNA processing, these precursors accumulate in serrate-1 mutants, facilitating their detection using standard RNA-Seq protocols. We first use the mapping of the RNA-Seq reads to the reference genome to annotate the potential primary transcripts of MIRNAs expressed in the embryo. We then quantify these pri-miRNAs in wild type and serrate-1 mutants. Finally, we use differential expression analysis to determine which are up-regulated in serrate-1 compared to wild type, to select the best candidates for bona fide pri-miRNAs expressed in the globular stage embryos. In addition, we analyze a previously published RNA-Seq dataset of wild type and dicer-like 1 mutant embryos at the globular stage [1]. Our data are interpreted and discussed in a separate article [2].

SUBMITTER: Lepe-Soltero D 

PROVIDER: S-EPMC5671514 | biostudies-literature | 2017 Dec

REPOSITORIES: biostudies-literature

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Annotating and quantifying pri-miRNA transcripts using RNA-Seq data of wild type and <i>serrate-1</i> globular stage embryos of <i>Arabidopsis thaliana</i>.

Lepe-Soltero Daniel D   Armenta-Medina Alma A   Xiang Daoquan D   Datla Raju R   Gillmor C Stewart CS   Abreu-Goodger Cei C  

Data in brief 20171012


The genome annotation for the model plant <i>Arabidopsis thaliana</i> does not include the primary transcripts from which <i>MIRNAs</i> are processed. Here we present and analyze the raw mRNA sequencing data from wild type and <i>serrate-1</i> globular stage embryos of <i>A. thaliana</i>, ecotype Columbia. Because <i>SERRATE</i> is required for pri-miRNA processing, these precursors accumulate in <i>serrate-1</i> mutants, facilitating their detection using standard RNA-Seq protocols. We first us  ...[more]

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